逆转录病毒载体的脐带血细胞转导:优化基因转移的临床前研究。

Blood cells Pub Date : 1994-01-01
M E Hanley, J A Nolta, R Parkman, D B Kohn
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引用次数: 0

摘要

人类脐带血(UCB)可以作为基因治疗的造血干细胞来源,作为异基因骨髓移植的替代品,用于治疗许多遗传疾病。为了确定产生最大的基因转移到UCB祖细胞的条件,我们检查了一些变量。我们使用传递新霉素(G418)抗性的无细胞逆转录病毒载体上清液,并测量G418抗性祖细胞衍生菌落的百分比。将逆转录病毒上清液添加到基础培养基中的UCB细胞中,每天1次,连续3天,与单独暴露于上清液(3.1%)相比,g418抗性菌落增加了3倍(9.8%)。为了确定重组人生长因子在转导过程中是否有益,我们比较了不同组合中白细胞介素-3 (IL-3)、IL-6和肥大细胞生长因子(MGF,一种c-kit配体)的存在。与在基础培养基中的转导相比,这三个因素共同导致基因转移增加了三倍(30.4%)。将UCB细胞在含有IL-3、IL-6和MGF的培养基中预培养3天后,在第4、5和6天加入逆转录病毒上清液,基因转移的平均程度为21.8%,而在第1、2和3天转导UCB细胞的平均程度为34.4%。在UCB细胞转导过程中骨髓基质的存在并没有进一步增加基因转移。我们得出结论,重组人生长因子IL-3、IL-6和MGF可以有效地转导UCB祖细胞,可能是基因治疗的合适来源。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Umbilical cord blood cell transduction by retroviral vectors: preclinical studies to optimize gene transfer.

Human umbilical cord blood (UCB) can be a source of hematopoietic stem cells for gene therapy, as an alternative to allogeneic bone marrow transplantation, for the treatment of a number of genetic diseases. To determine conditions that yield maximal gene transfer into UCB progenitor cells, we examined a number of variables. We used cell-free retroviral vector supernatants that convey neomycin (G418) resistance and measured the percentage of G418-resistant progenitor-derived colonies. Adding retroviral supernatant to the UCB cells in basal medium once a day for 3 days produced a threefold increase of G418-resistant colonies (9.8%) compared to a single exposure to supernatant (3.1%). To establish whether recombinant human growth factors are beneficial during transduction, the presence of interleukin-3 (IL-3), IL-6, and mast cell growth factor (MGF, a c-kit ligand) were compared in different combinations. Inclusion of the three factors together caused a threefold increase of gene transfer (30.4%) compared to transduction in basal medium. When the UCB cells were precultured in medium containing IL-3, IL-6, and MGF for 3 days before addition of the retroviral supernatant on days 4, 5, and 6, the average extent of gene transfer was 21.8%, compared with an average of 34.4% when UCB cells were transduced on days 1, 2, and 3. The presence of marrow stroma during the transduction of the UCB cells did not further increase gene transfer. We conclude that UCB progenitor cells can be efficiently transduced with the use of recombinant human growth factors IL-3, IL-6, and MGF and may be a suitable source for gene therapy.

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